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Immunogenicity of a new, inactivated canine adenovirus type 2 vaccine for dogs

机译:一种新的灭活的犬腺病毒2型犬疫苗的免疫原性

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Purpose We constructed a new canine adenovirus type 2 (CAV-2) vaccine candidate using the recently isolated Korean CAV-2 strain; we termed the vaccine APQA1701-40P and evaluated its safety and immunogenicity in dogs. Materials and Methods To generate the anti-CAV-2 vaccine, APQA1701 was passaged 40 times in MDCK cells growing in medium containing 5 mM urea and the virus was inactivated using 0.05% (volume per volume) formaldehyde. Two vaccines were prepared by blending inactivated APQA1701-40P with two different adjuvants; both were intramuscularly injected (twice) into guinea pigs. The safety and immunogenicity of the Cabopol-adjuvanted vaccine were evaluated in seronegative dogs. The humoral responses elicited were measured using an indirect enzyme-linked immunosorbent assay (I-ELISA), and via a virus neutralization assay (VNA). Results The new, inactivated CAV-2 vaccine strain, APQA1701-40P, lacked six amino acids of the E1b-19K protein. In guinea pigs, the Cabopol-adjuvanted vaccine afforded a slightly higher VNA titer and I-ELISA absorbance than an IMS gel-adjuvanted vaccine 4 weeks post-vaccination (p0.05). Dogs inoculated with the former vaccine developed a significantly higher immune titer than non-vaccinated dogs. Conclusion The Cabopol-adjuvanted, inactivated CAV-2 vaccine was safe and induced a high VNA titer in dogs.
机译:目的,我们使用最近孤立的韩国CAV-2菌株构建了一种新的犬腺病毒类型2(CAM-2)疫苗候选物;我们称之为疫苗APQA1701-40P,并在狗的安全性和免疫原性评估。产生抗COM-2疫苗的材料和方法,APQA1701在含有5mM尿素的培养基中生长的MDCK细胞中传代40次,并且使用0.05%(每体积体积)甲醛灭活病毒。通过用两种不同的佐剂混合灭活的APQA1701-40P来制备两个疫苗;两者都肌内注射(两次)进入豚鼠。在血清可养犬中评估了山波波辅助疫苗的安全性和免疫原性。使用间接酶联免疫吸附测定(I-ELISA)和通过病毒中和测定(VNA)来测量引起的液体反应。结果新的灭活CAV-2疫苗菌株APQA1701-40P缺少六种E1B-19K蛋白的六个氨基酸。在豚鼠中,碳波池佐剂疫苗得到稍高的VNA滴度和I-ELISA吸光度,而不是接种后4周的IMS凝胶佐剂疫苗(P> 0.05)。接种前疫苗接种的狗显着高于非接种疫苗的免疫滴度。结论碳波取辅助,灭活的CAV-2疫苗是安全的,诱导狗的高VNA滴度。

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